Cloning and expression analysis of litchi (Litchi Chinensis Sonn.) polyphenol oxidase gene and relationship with postharvest pericarp browning

Cloning and expression analysis of litchi (Litchi Chinensis Sonn.) polyphenol oxidase gene and relationship with postharvest pericarp browning

Polyphenol oxidase (PPO) plays a key role in the postharvest pericarp browning of litchi fruit, but its underlying mechanism remains unclear. In this study, we cloned the litchi PPO gene (LcPPO, JF926153), and described its expression patterns. The LcPPO cDNA sequence was 2120 bps in length with an...

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Veröffentlicht in:PloS one 2014-04, Vol.9 (4), p.e93982-e93982
Hauptverfasser: Wang, Jiabao, Liu, Baohua, Xiao, Qian, Li, Huanling, Sun, Jinhua
Format: Artikel
Sprache:eng
Schlagworte:
Agricultural biotechnology
Amino acid sequence
Analysis
Biochemistry
Biology and Life Sciences
Browning
Catechol Oxidase - biosynthesis
Catechol Oxidase - genetics
Cloning
Cloning, Molecular
Cultivars
Deoxyribonucleic acid
DNA
Enzymes
Fruit - enzymology
Fruit - genetics
Fruits
Gene Expression
Gene Expression Regulation, Plant
Genetic aspects
Genetic research
Litchi
Litchi - enzymology
Litchi - genetics
Litchi chinensis
Methods
Nucleotide sequence
Open Reading Frames
Organ Specificity
Oxidation
Packaging
Pericarp
Phenols
Phylogeny
Physical Sciences
Physiological aspects
Physiology
Plant Proteins - biosynthesis
Plant Proteins - genetics
Plastics
Polymerase chain reaction
Polyphenol oxidase
Polyphenols
PPOs
Sequence Homology, Amino Acid
Soapberries
Storage
Temperature
Water loss
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Zusammenfassung:Polyphenol oxidase (PPO) plays a key role in the postharvest pericarp browning of litchi fruit, but its underlying mechanism remains unclear. In this study, we cloned the litchi PPO gene (LcPPO, JF926153), and described its expression patterns. The LcPPO cDNA sequence was 2120 bps in length with an open reading frame (ORF) of 1800 bps. The ORF encoded a polypeptide with 599 amino acid residues, sharing high similarities with other plant PPO. The DNA sequence of the ORF contained a 215-bp intron. After carrying out quantitative RT-PCR, we proved that the LcPPO expression was tissue-specific, exhibiting the highest level in the flower and leaf. In the pericarp of newly-harvested litchi fruits, the LcPPO expression level was relatively high compared with developing fruits. Regardless of the litchi cultivar and treatment conditions, the LcPPO expression level and the PPO activity in pericarp of postharvest fruits exhibited the similar variations. When the fruits were stored at room temperature without packaging, all the pericarp browning index, PPO activity and the LcPPO expression level of litchi pericarps were reaching the highest in Nandaowuhe (the most rapid browning cultivar), but the lowest in Ziniangxi (the slowest browning cultivar) within 2 d postharvest. Preserving the fruits of Feizixiao in 0.2-μm plastic bag at room temperature would decrease the rate of pericarp water loss, delay the pericarp browning, and also cause the reduction of the pericarp PPO activity and LcPPO expression level within 3 d postharvest. In addition, postharvest storage of Feizixiao fruit stored at 4°C delayed the pericarp browning while decreasing the pericarp PPO activity and LcPPO expression level within 2 d after harvest. Thus, we concluded that the up-regulation of LcPPO expression in pericarp at early stage of postharvest storage likely enhanced the PPO activity and further accelerated the postharvest pericarp browning of litchi fruit.
ISSN:1932-6203
1932-6203
DOI:10.1371/journal.pone.0093982